Nucleotide sequences and proteins conferring cycloheximide resistance

ABSTRACT

The invention relates to cycloheximide resistance proteins, which are capable of conferring resistance to cycloheximide to cells containing the protein. The invention also relates to fragments or derivatives of cycloheximide proteins which confer cycloheximide resistance and/or are recognized by antibodies specific for the cycloheximide resistance proteins.

This is a division of application Ser. No. 08/175,388 filed on Jun. 9, 1994, now U.S. Pat. No. 5,645,674, which was filed as International Application No. PCT/FR92/00685 filed on Jul. 15, 1992.

BACKGROUND OF THE INVENTION

1. Field of the Invention

The invention relates to nucleotide sequences capable of conferring resistance to cycloheximide, cycloheximide resistance proteins and their use as selection markers, for example, to monitor nucleic acid transfer.

2. Description of the Related Art

The inventors have, in fact, investigated selectionmarkers suitable for monitoring nucleic acid transfer in eukaryotes, markers which might be more efficient than the markers usually used which are derived from prokaryotic organisms. It is know for example that the markers usually used (geneticin G-418, hygromycin and bleomycin) are derived from resistance genes isolated from prokaryotes and are usually rather inefficient, particularly in fungi. These problems oblige experimenters to use very high concentrations of antibiotics which cause toxicity problems and increase production costs. Consequently, other selection agents have been used, for example selection by methotrexate, selection by auxotrophy, etc. However, these selection agents are not generally applicable. There is thus a need for the creation of systems suited to the use of a more efficient and/or potent marker than the markers known hitherto and at lower production costs.

Cycloheximide might constitute a potentially useful marker for example for detecting the transfer of heterologous nucleic acid in eukaryotes. For this purpose, the eukaryotes which it is desired to modify in a controllable manner by means of a detection test for resistance to cycloheximide, must be made resistant to this antibiotic under satisfactory conditions in order to ensure reliable monitoring of the transfer of a heterologous nucleic acid made either for research purposes or for the purpose of industrial exploitation.

Cycloheximide is an antibiotic which inhibits protein synthesis by binding to the 60S ribosomal subunit as described by STOCKLEIN et al. (1980, Curr. Genetics 1, 177-183).

Eukaryotic organisms naturally resistant to cycloheximide are rare; up to now observations relating to the mechanisms of resistance have been described in a mutant of an organism naturally sensitive to cycloheximide, the cyh2 mutant of the yeast Saccharomyces cerevisiae. In this context, the phenomenon of resistance is created by a modification of the ribosomal protein L29 (STOCKLEIN et al., 1980).

These mutant cellular organisms are usually resistant to low concentrations of cycloheximide (of the order of 5-10 μg/ml).

Other authors (TAKAGI et al. in the U.S. Pat. No. 4,857,460) have reported results relating to the study of resistance to cycloheximide in another yeast Candida maltosa. They present a DNA sequence conferring resistance to cycloheximide on C. maltosa. However, neither gene nor open reading frame was identified in this sequence. In other words, the U.S. Pat. No. 4,857,460 does not give the elements for the characterization of a gene, elements which could have led to a definition of the conditions for its use, for example, to transform eukaryotes different from Candida maltosa into strains resistant to cycloheximide in a reproducible manner.

SUMMARY OF THE INVENTION

The inventors have concerned themselves with the yeast Kluyveromyces lactis (K. lactis) and demonstrated the fact that cycloheximide resistance in K. lactis depends on the expression of a specific gene. They have also identified the fact that the level of resistance of this yeast to this antibiotic involves other elements linked to the presence of a specific DNA which has the role of cofactor (or cofactor sequence).

In an advantageous embodiment of the invention, the resistance obtained is specific for cycloheximide, the transformed hosts resistant to this antibiotic (cyc^(R)) being sensitive to several classical inhibitors of ribosomal functions (cryptopleurin, blasticidin, trichodermin, anisamycin, hygromycin).

Thus the inventors obtained in K. lactis a nucleic acid sequence of about 5.2 kb, capable of conferring a level of resistance to a cell host transformed by this sequence sufficiently high for the creation of a selection system as a result of resistance to this antibiotic, this resistance being expressed at a cycloheximide concentration higher than 1 mg/ml.

Within this nucleic acid sequence the inventors have identified and characterized a specific gene coding for a protein whose presence proves to be necessary for inducing the phenomenon of resistance in K. lactis.

This specific gene codes for a ribosomal protein which is responsible for resistance to a cycloheximide concentration of the order of 100 μg/ml. Complete resistance to this antibiotic in K. lactis requires not only the presence of this resistance-inducing sequence but also the presence of additional DNA elements contained in the 5.2 kb nucleic acid sequence defined by the inventors and described hereafter. These additional elements play the role of cofactors.

Thus, the subject of the present application is nucleotide sequences as well as a protein which are capable of conferring cycloheximide resistance an a eukaryote cell host naturally sensitive to this antibiotic or resistant to a low concentration of this antibiotic (also designated as low-level resistant organism). This first type of protein will be designated in what follows by the expression "resistance protein".

The invention also relates to a nucleic acid sequence comprising a gene which codes for the resistant protein described above in K. lactis, as well as sequences determining the presence of cofactors implicated in the level of resistance conferred by the above-mentioned protein.

It also relates to the gene coding for the resistance protein and the different nucleic acid fragments determining the presence of the cofactors.

It also relates to cloning and/or expression vectors for these nucleotide sequences as well as eukaryotic cell hosts transformed by these vectors.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 depicts plasmid pEMBL Ye23, a shuttle vector for E. coli and S. cerevisiae, into which the genomic library of K. lactis strain 2359-152 was inserted.

FIG. 2 depicts a sequence fragment of the DNA of K. lactis conferring cycloheximide resistance (SEQ ID NO:3).

FIG. 3 depicts a restriction map of the 5.2 kb DNA fragment of K. lactis which was inserted at the BamHI site of vector Ye23.

FIG. 4 depicts the sequence of the protein conferring cycloheximide resistance encoded by K. lactis DNA.

DESCRIPTION OF THE PREFERRED EMBODIMENTS

A first protein according to the invention or cycloheximide resistance protein is a protein whose presence is necessary and sufficient to confer resistance to cycloheximide on a host naturally sensitive to it. It is characterized in that it corresponds to the following amino acid sequence A (SEQ ID NO: 1), or in that it comprises all or part of this sequence A (SEQ ID NO: 1), possibly modified, provided that the protein formed confers cycloheximide resistance on a recombinant eukaryotic host transformed by the nucleotide sequence coding for this protein under conditions allowing its production. ##STR1##

The property of this protein to confer cycloheximide resistance can be evaluated when it is produced in a specific eukaryotic cell host, naturally sensitive to cycloheximide at concentrations higher than a threshold defined as a function of the nature of the host, and when it allows resistance to be produced in this host at a concentration about 5 to 15 fold higher, and preferably about 10 fold higher, than the cycloheximide concentration conferring the natural sensitivity in this host.

In yeasts, in S. cerevisiae in particular, this increase in the resistance level is about 10 fold, even 100 fold to 1000 fold higher than the level observed in the wild type strain.

As examples, the order of magnitude of the natural sensitivity of various organisms to cycloheximide is given below:

yeasts S. cerevisiae: 1 μg/ml

higher eukaryotic cells: 1 μg/ml

tobacco plants: 10 μg/ml.

Generally, the natural sensitivity of a specific organism is expressed as soon the presence of cycloheximide in the culture medium inhibits the growth and multiplication of the organism

When reference is made in this text to a eukaryotic host sensitive to cycloheximide, this reference must be interpreted as designating any eukaryotic organism complying with the above definition in regard to cycloheximide resistance.

A cycloheximide resistance protein according to the invention may also be characterized in that it is encoded in the following nucleotide sequence ID NO:2, by a part of sequence ID NO:2 or by a modified sequence ID NO:2, provided that the protein encoded by the partial sequence or this modified sequence is capable of conferring resistance to a concentration equal to at least 100 μg/ml of cycloheximide when it is introduced in a eukaryotic host, for example the yeast Saccharomyces cerevisiae under conditions allowing its expression ##STR2##

The invention also relates to a nucleic acid sequence comprising the sequence coding for the cycloheximide resistance protein in K lactis, this protein being characterized in that it complies with one of the following definitions:

(a) it is a nucleic acid sequence of K. lactis of about 5.2 kb capable of conferring cycloheximide resistance to a concentration higher than 1 mg/ml in K. lactis or in S. cerevisiae, and comprising the restriction sites defined in FIG. 3. The various sites are situated at the following positions:

Sau3A: 0, StuI: +300 bp, PvuII: +600 bp, BglIII: +900 bp, BstXI: +1200 bp, PvuII: +2300, PstI: +2400 bp, PstI: +3000 bp, EcoRI: +3200 bp, HindIII: +3300 bp, EcoRI: +3700 bp, HindIII: +4500 bp, HindIII: +4540 bp, SalI: +5100 bp.

(b) it is a nucleic acid sequence of about 5.2 kb, comprising nucleotide sequence ID NO:2 or hybridizing with the sequence complementary to sequence ID NO:2 under conditions of high stringency (0.1×SSC, 0.1% SDS at 65° C.), and capable of conferring resistance to a cycloheximide concentration higher than 100 μg/ml, and preferably higher than 1 mg/ml, in K. lactis;

(c) it is a nucleic acid sequence of about 5.2 kb, comprising the following nucleotide sequence ID NO:3 or hybridizing with the sequence complementary to sequence ID NO:3 under conditions of high stringency, and capable of conferring resistance to a cycloheximide concentration higher than 100 μg/ml, and preferably higher than 1 mg/ml, in K. lactis;

(d) it is a nucleic acid sequence comprising the nucleotide sequence situated between positions 9 and 2763 of sequence ID NO:3 or a sequence hybridizing with the sequence complementary to sequence ID NO:3 under conditions of high stringency, and capable of conferring resistance to a cycloheximide concentration higher than 100 μg/ml, and preferably higher than 1 mg/ml, in K. lactis. When a nucleic acid sequence complying with one of the definitions given above is introduced into a yeast such as S. cerevisiae, it confers on this yeast resistance to cycloheximide at a concentration higher than 100 μg/d, this being advantageously expressed for a cycloheximide concentration higher than 1 mg/ml. ##STR3##

According to a preferred embodiment of the invention, the two DNA sequences defined under points (b) and (c) above correspond in addition to the restriction map given in FIG. 3.

According to another preferred embodiment of the invention, the nucleic acid sequence described above is extracted from the E. coli strain DH5γ recombined with the plasmid Ye23/31, deposited with the CNCM (Collection Nationale de Culture de Microorganismes Institut Pasteur, 25, rue du Docteur Roux, 75724 Paris Cedex 15, France) in Paris, France in 2, Jul. 1991 under number 1-1121.

In this context "complementary sequence" to a given nucleic acid sequence is said to be a reverse and complementary sequence to a given nucleotide sequence. The term "reverse" takes into account the restoration of the 5'-3' orientation of the nucleic acid which is also complementary to the given base sequence by the nature of the nucleotides it contains.

The 5.2 kb nucleic acid sequence comprises in addition to the sequence coding for the said resistance protein described above, the DNA which may be designated by the term "cofactor", which determines the level of resistance to cycloheximide in K. lactis and in a cell host transformed by this sequence. This cofactor DNA is included in sequence ID NO:3.

Thus the invention also relates to the following DNA fragments, included in the 5.2 kb sequence described above:

the BamHI (5')--PvuII (3') fragment of about 2.3 kb

the PvuII (5')--SalI (3') fragment of about 3 kb.

The production of cycloheximide resistance in a given cell host at a defined level can be achieved by transforming this host with a nucleic acid coding for the cycloheximide resistance protein and with a cofactor DNA fragment present in the 5.2 kb sequence, adjacent or not adjacent to the above nucleic acid, the introduction of this fragment in the host being directly correlated with the level of resistance observed. One embodiment of the transformation of a cell host is described in the following pages.

The resistance protein can be isolated by lysis of the K. lactis cells followed by the steps described in "The Yeasts" (second edition by A. H. Rose and J. S. Harrison, vol. 4: 504-505).

The purification can also be done by affinity using antibodies directed against the sequence A. In this case an over-expression of the ribosomal protein is produced which is then purified on polyacrylamide gel according to standard techniques. The molecular weight band corresponding to the sequence A protein is excised. This band is the major band because it results from the over-expression of the protein. It is subjected to reaction with the antibodies, in particular monoclonal antibodies, described above, produced according to standard procedures.

The invention also relates to the ORF A sequence containing nucleic acid I (SEQ ID NO:2), ORF A being itself included between the nucleotides at positions 1 and 1560 of sequence ID NO:3, it being understood that the sequence included between nucleotides 633 and 1222 corresponds to the intron V. The ORF A sequence contains two exons, one being formed by the nucleotides ATGG situated between nucleotides 629 and 632, the other exon being formed by the sequence included between nucleotides 1223 and 1539.

The nucleotide sequence included between nucleotides 1 and 1539 contains the promoter for the gene, in addition to the ORF A sequence.

Other particularly useful nucleotide sequences in the framework of the invention are the following sequences:

the nucleotide sequence ORF A as such or any nucleotide chain which hybridizing with the sequence complementary to ORE A under the following conditions: 60° C., 2×SSC 5×Denhart, 0.1% SDS, 0.1 mg/ml salmon sperm DNA,

the coding sequence ID NO:2 (or exon) contained in the ORF A nucleic acid which codes for the resistance protein in Kluyveromyces lactis, and included between nucleotides 629 and 1539, which forms a sequence of two exons one of which is included between nucleotides 629 and 632 and the other between nucleotides 1223 and 1539,

the sequence IV, comprising nucleotides 1561 and 2740 and which corresponds to the so-called cofactor sequence situated between nucleotides 1540 and 2763 and capable of increasing the cycloheximide resistance conferred by the resistance protein,

the intron V of ORF A,

the nucleotide sequence III defined by nucleotides 1 and 628, and more particularly by 8 and 628, which contains the regulatory elements of expression for ORF A and in particular the promoter region for the transcription of the ORF A sequence; this promoter contains in particular regulatory regions of the promoters for proteins characteristic of the ribosomes, regions of the "UAS_(RPG) " type such as described by W. H. Mager (Biochern Biophys. Acta (1988) 949: 1-15). These so-called ribosomal proteins are imported into the nucleus of the cell which produces them, where they are assembled into ribosomes,

the so-called cofactor sequence IV included between nucleotides 1561 and 2740 which is capable of increasing the resistance to cycloheximide conferred by the resistance protein.

The subject of the invention is also recombinant vectors in particular for cloning and/or expressing the proteins previously characterized.

These expression vectors are characterized by the incorporation, at one of their sites inessential for their replication, of a nucleotide sequence selected from those previously mentioned under the control of the regulatory elements necessary for its expression in a selected eukaryotic cell host, these regulatory elements comprising in particular an optionally inducible promoter and a transcription termination sequence.

Such a vector may comprise a nucleotide sequence coding for a protein called cycloheximide resistance protein, alone or in association with a cofactor nucleotide sequence complying with the previously given definition.

In addition, the invention relates to vectors complying with the above definitions characterized in that they contain in addition a specific heterologous nucleic acid, for example a nucleic acid coding for a protein of industrial or pharmaceutical interest, this nucleic acid being under the control of regulatory elements necessary for its expression in the host, these elements being possibly fused with the sequences controlling the transcription of the nucleotide sequences involved in cycloheximide resistance.

The resistance system according to the invention makes it possible to monitor advantageously the insertion of heterologous sequences such as that of human serum albumin, the surface antigen of hepatitis B virus, with a view to their expression in a eukaryotic host.

As examples, it is possible to use vectors of the replicating plasmid type, integrative vectors such as pSVL (Pharmacia). Such a vector may, for example, contain the nucleotide sequence coding for the protein corresponding to sequence A (SEQ ID NO:1) without its intron.

Generally, it is useful for the implementation of the invention to use multiple-copy vectors, in particular when the transformed cells are eukaryotic cells.

Preferred vectors according to the invention are vectors suited for expression in yeasts, in particular of industrial importance, which it is desired to label with a resistance marker, for example when a auxotrophic marker is not available, a particular yeast being Pichia pastoris or S. pombe, or vectors suited for expression in a higher eukaryotic animal cell, for example baculovirus, or also vectors suited for expression in a plant cell such as tobacco plants. Thus simian cells or murine cells may be transformed.

A particularly advantageous vector in the framework of the invention is the plasmid Ye23/31 which transforms the E. coli strain DH5γ deposited with the CNCM on 2 Jul. 1991 under the number I-1121.

Furthermore, the invention relates to a eukaryotic cell characterized in that it is transformed by a vector corresponding to the above characteristics and in particular in that it is a yeast cell, for example Pichia pastoris, a higher eukaryotic animal cell, for example an insect cell or a mammalian cell, in particular a murine or simian cell, a human cell or also a plant cell.

Such a recombinant cell may be obtained by all of the procedures for the insertion of heterologous sequences commonly used for the preparation of recombinant cell host. It is possible in particular to apply the electroporation procedure described by M. Becker, L. Garente in Methods in Enzymology (1991 vol. 194: 182-187).

It will also be possible to have recourse to the procedures described in the patent application WO 84/02913 on the subject of the insertion in to plant cells of nucleotide sequences heterologous with respect to the nucleic acids naturally contained in such cells.

As an application, the resistance proteins previously described can be used in a selection system corresponding specifically to a cycloheximide-type marker in order to monitor the introduction into a eukaryotic host of a heterologous sequence which it is desired to express in this host. The selection will be the easier if the resistance can be verified with a high concentration of antibiotic, this resistance then resulting from the association of the above resistance protein with a cofactor previously defined.

It is particularly interesting in the framework of the invention to prepare proteins which make it possible to obtain resistance at a cycloheximide concentration of about 100 μg/ml, even 1 mg/ml.

Furthermore, the invention relates to a procedure for monitoring the presence of a heterologous nucleic acid in a cell host, characterized in that it comprises:

the transformation of the cell host by an expression vector containing at one of its sites inessential for its replication the heterologous nucleic acid, on the one hand, a nucleotide sequence coding for a resistance protein, on the other, and optionally a cofactor nucleotide sequence under the control of the regulatory elements necessary for the expression of these sequences in a selected cell host,

the culture of the cell host thus transformed,

the placing of the host in contact with a defined concentration of cycloheximide and the detection of host resistance to this antibiotic.

The subject of the invention is also a method for obtaining cells which express cycloheximide resistance as described in the preceding pages, characterized by the following steps:

transformation of a given cell host by a nucleic acid sequence of the invention inserted beforehand in a host plasmid under conditions allowing the expression of the above-mentioned nucleic acid sequence;

culture of the transformed cells (transformants) in a complete medium containing a very low cycloheximide concentration, preferably lower than 2 μg/ml;

recovery of the resistant strains at a cycloheximide concentration higher than 1 to 10 μg/ml.

As an example, in respect to yeasts, the steps described above are performed under the following conditions:

the culture of the transformants is carried out at a temperature between about 29° C. and about 30° C., preferably 30° C., in the presence of a cycloheximide concentration lower than 2 μg/ml for 12 to 36 hours,

the strains selected from this culture are those which are resistant culture in the presence of 100 μg/ml of cycloheximide,

the complete culture medium contains 10 g/l of yeast extract, 20 g/l of Bacto peptone and 20 g/l of glucose.

The culture step of the transformants mentioned above is preferably carried out for 12 to 18 hours at 30° C., after transformation in a complete liquid medium at sub-limiting concentrations (1 μg/ml). This concentration may be adapted as a function of the strain and the species of yeast used.

In the case of eukaryotic cells as for example (mouse) LTK-cells, the culture medium may be Dulbecco medium supplemented with 10% newborn calf serum and by a fungicidal antibiotic.

The recombinant clones are selected according to the procedure described by Delpeyroux et al. in Journal of Virology (Dec. 1990 vol. 64 (12): 6090-6100).

In summary, the cells are cotransfected with 10 times more recombinant plasmid than vector containing the antibiotic resistance gene G418 (Colbere--Garapin F. et al. 1981, J. Mol. Biol. 150: 1-14). After three weeks, the resistant clones are placed in a culture medium supplemented with cycloheximide at a concentration of 1 to 10 μg/ml.

When the cell host is S. cerevisiae, the plasmid containing the nucleotide sequence of the invention may be an episomal multi-copy plasmid of the YEp plasmid family, for example the 2μ plasmid of S. cerevisiae, or the episomal multicopy plasmid Ye 23/31.

Other advantages and characteristics of the invention will became apparent from the Examples and Figures which follow.

FIG. 1: cloning vector containing the DNA fragment of K. lactis of about 5.2 kb conferring cycloheximide resistance.

A genome library of the K. lactis strain 2359-152 resistant to several mg/ml of cycloheximide was constructed. This library is constructed in a shuttle vector E. coli/S. cerevisiae: pEMBL Ye 23 (Baldari et al. 1985 Gene 35: 27-32, FIG. 1). The chromosomal DNA of K. lactis was partially digested by the enzyme Sau3A, then fractionated on a sucrose gradient. The fractions containing DNA included a size between 4 and 9 kb were recovered and the DNA was ligated to the vector YE 23 previously cut and dephosphorylated at the BamHI site situated in the beta-galactosidase gene. This ligation mixture made it possible to transform the E. coli strain XL1 and the recombinant transformants were selected on a medium which allows an insertion in the beta-galactosidase gene to be visualized. 23000 recombinant E. coli clones were thus selected. Restriction analysis of the plasmids of fifty clones enabled the mean size of the DNA insertion in K. lactis to be estimated at 5 kb, which gives a 99.5% probability of obtaining a specific gene.

E. coli strain XL1 (strain developed by the Stratagene company): endA1, hsdR17 (rk⁻, mk⁺), supE44, thi⁻, λ⁻, recA1, gyrA96, relA1, Δ (lac), F, proAB, laciq Z M15, Tn10 (tet^(r)).

S. cerevisiae strain OL1: γ, leu2-3, leu2-112, his3-11, his3-15, ura3-251, ura3-273.

FIG. 2: Sequence fragment of the DNA of K. lactis conferring cyeloheximide resistance (sequence II ID NO:3).

FIG. 3: restriction map of the 5.2 kb DNA fragment of K. lactis which was inserted at the BamHI site of the vector Ye 23 (C. Baldari et al., Gene (1985) 35: 27).

The sequenced SalI-PvuII fragment (2.8 kb) contains the ribosomal protein. The various sites are situated respectively at the following positions:

Sau3A: 0, StuI +300 bp, PvuII: +600 bp, BglIII: +900 bp, BstXI: +1200 bp, PvuII: +2300, PstI: +2400 bp, PstI: +3000 bp, EcoRI: +3200 bp, HindIII: +3300 bp, EcoRI: +3700 bp, HindIII: +4500 bp, HindIII: +4540 bp, SalI: +5100 bp.

FIG. 4 (SEQ ID NO:1): Protein conferring cycloheximide resistance, encoded in K. lactis DNA.

EXAMPLES I-Cloning at the DNA fragment of K. lactis conferring cycloheximide resistance I.1) Construction of a K. lactis library in S. cerevisiae:

A genome library of the K. lactis strain 2359-152 (WESOLOWSKI et al., 1982, Curr. Genetics 5: 191-197) resistant to concentrations of several mg/ml of cycloheximide was created. This library was constructed in a shuttle vector E. coli/S. cerevisiae: pEMBL YE 23 (BALDARI et al., 1985, Gene 35: 27-32) (FIG. 1). K. lactis chromosomal DNA was partially digested by the enzyme Sau3A, then fractionated on a sucrose gradient. The fractions containing DNA of a size included between 4 and 9 kb were recovered and ligated to the vector YE 23 previously cut and dephosphorylated at the BamHI site situated in the beta-galactosidase gene. This ligation mixture made it possible to transform the E. coli XL1 strain (BULLOCK et al., 1987, Biotechniques 5, 376-379) and the recombinant transformants were selected on a medium which allows an insertion in the beta-galactosidase gene to be visualized. 23000 recombinant E. coli clones were thus selected. Restriction analysis of the plasmids of fifty clones enabled the mean size of the DNA insertion in K. lactis to be estimated at 5 kb, which gives a 99.5% probability of obtaining a specific gene.

I.2) Transformation of S. cerevisiae and production of cycloheximide resistant transformants:

The S. cerevisiae strain OL1 (BOY-MARCOTTE et al., 1982, Gene 20: 433-440), sensitive to cycloheximide concentrations lower than 1 μg/ml, was transformed with the DNA extracted from the library. In a first stage, the transformants were screened for uracil prototrophy which enabled the total number of transformants to be evaluated. In a second stage these transformants were subcultured on a medium containing cycloheximide at two concentrations: 10 and 100 ug/ml. 3500 URA⁺ transformants were obtained, 7 of which are resistant to cycloheximide concentrations higher than 100 ug/ml. After analysis, it emerged that 6 of the 7 clones retained had integrated the DNA derived from K. lactis in to their genome. However, in the seventh transformant the resistance character was maintained on the Ye 23/31 plasmid derived from the pEMBLYe23 vector. This transformant is resistant to very high cycloheximide concentrations, in excess of 1 mg/ml. The DNA fragment conferring cycloheximide resistance is about 5.2 kb.

Furthermore, for the transformants which have integrated the K. lactis DNA fragment into their genome, the resistance phenomenon is maintained in a diploid, heterologous for this marker. The "cycloheximide resistant" character is thus dominant.

I.3) Protein responsible for cycloheximide resistance

This entire fragment was inserted into pBluescript phagemid vectors (Stratagene). Different unidirectional deletions were constructed with the aid of the enzyme couple ExoIII/S1. The sequencing of the single-stranded DNA was carried out with the aid of the Sanger procedure by using universal primers or primers synthesized in the laboratory from the sequence itself.

A fragment of the sequence thus obtained is shown in FIG. 2. It contains in particular an open reading frame ORF A.

ORFA:

This Open reading frame is 320 bp long (FIG. 2) and carries an intron of 590 bp. This intron is located at the 5' end of the gene, after the first base after the ATG. The protein encoded by the exon contains 150 amino acids (FIG. 4, SEQ ID NO:1). The search for homologies with the aid of the EMBL and GENEBANK data banks shows that the ORF A has a 75% homology at the amino acid level with the ribosomal protein L36a of the rat (GALLAGHER et al., 1988, DNA 7: 269-273) and 74% homology with a human ribosomal protein (DAVIES et al., 1986, Gene 45: 183-191) which is itself homologous with the ribosomal protein rp44 (also designated L41) of S. cerevisiae (ITOH, 1978 FEBS Lett. 96: 399-402).

This sequence is sufficient to confer a high level of cycloheximide resistance; however, this level is lower than that observed in the transformants possessing the initial 5.2 kb fragment.

I.4) Expression of the open reading frame A:

In order to determine to what extent the so-called resistance protein is responsible for the cycloheximide resistance phenomenon, the same S. cerevisiae strain was transformed under the same conditions with a vector containing only the ORF A. The transformants which possess the ORF A are resistant to cycloheximide However, the level of resistance observed (100 μg/ml) is about ten times lower than that obtained when the ORF A is associated with the cofactor DNA contained in the entire fragment of 5.2 kb (1000 μg/ml). On the other hand, the deletion of the ORF A sequence leads to the abolition of resistance.

Conclusions:

A gene responsible for the phenomenon of cycloheximide resistance was isolated from a DNA fragment of K. lactis. This system is composed of a ribosomal protein (ORF A) very closely analogous to the human L36a and rat ribosomal proteins as well as to rp44 (or L41) of S. cerevisiae. This protein is necessary to cause the phenomenon if resistance but is not sufficient to have complete resistance to the antibiotic The presence of a cofactor located on the cloned 5.2 kb fragment of K. lactis is necessary to obtain resistance at about the 1 mg/ml level in K. lactis.

    __________________________________________________________________________     SEQUENCE LISTING                                                               (1) GENERAL INFORMATION:                                                       (iii) NUMBER OF SEQUENCES: 3                                                   (2) INFORMATION FOR SEQ ID NO:1:                                               (i) SEQUENCE CHARACTERISTICS:                                                  (A) LENGTH: 106 amino acids                                                    (B) TYPE: amino acid                                                           (C) STRANDEDNESS: single                                                       (D) TOPOLOGY: unknown                                                          (ii) MOLECULE TYPE: protein                                                    (xi) SEQUENCE DESCRIPTION: SEQ ID NO:1:                                        MetValAsnValProLysThrArgLysThrTyrCysLysGlyLysGlu                               151015                                                                         CysArgLysHisAlaGlnHisLysValThrGlnTyrLysAlaGlyLys                               202530                                                                         AlaSerLeuTyrAlaGlnGlyLysArgArgTyrAspArgLysGlnSer                               354045                                                                         XaaPheGlyGlyGlnThrLysGlnIlePheHisLysLysAlaLysThr                               505560                                                                         ThrLysLysValValLeuArgLeuGluCysMetSerCysLysThrLys                               65707580                                                                       ThrGlnLeuAlaLeuLysArgCysLysHisPheGluLeuGlyGlyGlu                               859095                                                                         LysLysGlnLysGlyGlnAlaLeuGlnPhe                                                 100105                                                                         (2) INFORMATION FOR SEQ ID NO:2:                                               (i) SEQUENCE CHARACTERISTICS:                                                  (A) LENGTH: 321 base pairs                                                     (B) TYPE: nucleic acid                                                         (C) STRANDEDNESS: unknown                                                      (D) TOPOLOGY: unknown                                                          (ii) MOLECULE TYPE: DNA (genomic)                                              (xi) SEQUENCE DESCRIPTION: SEQ ID NO:2:                                        ATGGTTAACGTTCCAAAGACCAGAAAGACTTACTGTAAGGGTAAGGAGTGCCGTAAGCAC60                 GCCCAACACAAGGTTACCCAATACAAGGCTGGTAAGGCTTCCTTGTACGCTCAAGGTAAG120                AGAAGATATGACCGTAAACAATCTGGTTTCGGTGGTCAAACCAAGCAAATTTTCCACAAG180                AAAGCTAAGACTACCAAGAAGGTCGTTTTGAGATTGGAATGTATGTCCTGTAAGACCAAG240                ACCCAATTGGCTTTGAAGAGATGTAAGCACTTCGAATTGGGTGGTGAAAAGAAGCAAAAG300                GGTCAAGCTTTGCAATTCTGA321                                                       (2) INFORMATION FOR SEQ ID NO:3:                                               (i) SEQUENCE CHARACTERISTICS:                                                  (A) LENGTH: 2842 base pairs                                                    (B) TYPE: nucleic acid                                                         (C) STRANDEDNESS: double                                                       (D) TOPOLOGY: unknown                                                          (ii) MOLECULE TYPE: DNA (genomic)                                              (xi) SEQUENCE DESCRIPTION: SEQ ID NO:3:                                        CCTCGAGGTCGACATTCAAGGGTTTAGTATCCTGAAAACAAAGCTTGTATAGACAGCCGA60                 CGGTTCTTGGTGACTGTTTGCATCCGTGCACCATAAAATCTCTCTTAACCACCCACACAT120                TGATTTTCGTGTTCAATTGAAATGTGAAAAATAAAATTGTTTCCCAATTAGGACTATATT180                CGTCTGTGGGAAAATAACATTGCCTAGTGGCATTGGTGTGGCCTAACCAGGCCGAATCAC240                TCACTTTCCACTAACAGACCTTCCTCCTGGTCGGTCTGGTCTGGGCTACCGGCAGTGTAG300                TCTCTCTTGCCAACACATTACGCATTCATGCTTGCTTCTGCCTACTGCTTCCCCGCCCAG360                GCTAAGCTTGGACGTGCGTAGTCGGGGGGCCAGTAACGCCTGCTCGTCTGGACTTGTTCG420                CCTTCACTCTTGCTGCCGTCTCTGCTTCGATGGCTGCCATTCGGCAATTCTCATCTGGAA480                GGATTGAACCACCTTGAATTTTTCAACATTAAAATATTACACAAGGAAAGTTCATCATAG540                TAGATATATCGTATAGTTGATTGTTATAGCACCTATTTGTTTCAGTACATTCAGAAAGCG600                TAACTCAACAGAGATCAAATGAGTCACAATGGGTATGTGAACAAGATTTAAAATATACCG660                TGGAGATTGTCAGTGGTTTATTCGATTTTTGGTATCCTGAGGGAAGAATGGAACGTTTGA720                AGTTTAGTACCAAGTGAACATGAAATGAGCTATGGTTATTTAACAGAATACAGCATTTCA780                GAGTGAATCAATGAGAAAACACCAACCGTATTGGAAATTCAGATATTGCATCGACAAGGG840                GGGAGAGTTCATTTGAGTTGGTGAACTATATCAAAAGATCAGTATTTTGGTCGAAGTATG900                GACGATTCACTAGCATAAAACCCTGTTCACGCTGGAGGAAGTAATTTGGGTTATTTGTTG960                TCCCTATGTTTCTTAATTCGGTGTAGTCGAGACAACCTCAGAGAATTGTATATCAGTGAA1020               GTCAACGCTACACTGACTGAACATAATTAACAGGAACTCAGTCGTATTAAACAACTGGGG1080               TTCAGATAGCCTGGACCTCCCTATACAATAAGAAGAAGAGAATAGAATTCCTGCAATCAA1140               AATAAGCTGGATGAAGCTAAAGAATATTTTTTTACTAACATCGACATGTATCACTATCTT1200               ATGATATGTTAATTTCTAACAGTTAACGTTCCAAAGACCAGAAAGACTTACTGTAAGGGT1260               AAGGAGTGCCGTAAGCACGCCCAACACAAGGTTACCCAATACAAGGCTGGTAAGGCTTCC1320               TTGTACGCTCAAGGTAAGAGAAGATATGACCGTAAACAATCTGGTTTCGGTGGTCAAACC1380               AAGCAAATTTTCCACAAGAAAGCTAAGACTACCAAGAAGGTCGTTTTGAGATTGGAATGT1440               ATGTCCTGTAAGACCAAGACCCAATTGGCTTTGAAGAGATGTAAGCACTTCGAATTGGGT1500               GGTGAAAAGAAGCAAAAGGGTCAAGCTTTGCAATTCTGAGATTATCTTTTGGAAGACCAT1560               TTGTTACCAATTTGTCAATTTTTTAACTTTTCTATAAGTATTACGAATTCACATATACTC1620               TTTCATCACATTTATAATCTCATATCTGTCATTTGTATAGTTTAGTCTCCACTGGGTACT1680               TCTTCACTTTGCGATTTGTATTATACGTATTCTAAGTATAATTTTCAGCAGAACGCATAA1740               GAGTTTATTAACAAGAATTGTTTACAAAGAATAGCGTAGGACTCAGGCTACATTATTGAT1800               CCTGCAGGCAGTAAAGCTTACATATGACCTTAGCTAATATAACATGTACATACTCACCAT1860               GTATACCACTTTTTTCATTCCATTGTCTAAAATATGTTTTCAATATTTGCCAAAATCGCC1920               AATTTCATTGGAAAAACAAAAACATCGAATCAAACTTGTTTTAGAAAACAACGAACATGA1980               AACTATACTGTTAACGTTTAGAGACATATTTCACGTCAACAAGGCCGTTTGGACGTCGCT2040               ACTTCAGCAACAACACGTAATGTACGGTGGATATTCGAATCAGAACTACTATCAACAGCC2100               TTCTGGTCGTCCGAAACGATTTTCAGCAACAGGGAAACATGCCCTTTTCGGAACCTTCTC2160               AGCCCATGTTCAGCACCAATTATATGAAACAACAAGGATCACAGCCGTCTTACAAGACCG2220               TCTGACCCAACAGCAATCGCAACCTCAGTCGCATAATAATCAATATTATCCGAATGGAGG2280               GTTTACTGATGTGCCCAACTTGAATTATCCAGCGACTCCACCACCAACTCAAAGCATTTA2340               TTCACATAACAACAACTCTAATTCGAAGGTATATCAATCCGCTCAGCATACATCTCCCGG2400               TCAATATTCTGTTGCCAGTGAGTCCGGTTTGTACATCCCGCCACCACTGCAGCAACAGCA2460               GAATGGTCAACAGAGTCCTGTGAGATCGGTACATCAACAGACACAGCAAACACCGCCAAC2520               ATTTACTCAGCAACAAAGCTCTTCCCAACCTCAGTCACCTCAACACAATACGTTATCATG2580               CACAGCAGCAGCAGCAGCAGCAGCAGCAGCAACAACAAACTCAACAGGCCCAGCAGCAAG2640               GACAACGACAAACTCAGCAACAGTCTCAGCAGCAAGCTCAACAACAGAATGGATCGGCGA2700               ATAATTACATGTATTTTGAGAGAAGACCTGACCTATTGACCAAAACTACCCAAGACAAAG2760               CAGATCGAATTCCTGCAGCCCGGGGGATCCACTAGTTCTAGAGCGGCCGCCACCGCGGTG2820               GAGCTCCAATTCGCCCTATAGT2842                                                     __________________________________________________________________________ 

We claim:
 1. A purified cycloheximide resistance protein comprising SEQ ID NO: 1, or fragments thereof, provided that said protein or fragment thereof confers resistance to cycloheximide at a concentration higher than or equal to 100 μg/ml on a recombinant eukaryotic host cell transformed by a nucleotide sequence coding for the protein, under conditions allowing for production of said protein.
 2. A purified cycloheximide resistance protein encoded by one of the following sequences:(1) SEQ ID NO:2; (2) a fragment of SEQ ID NO:2; or (3) a sequence which hybridizes to a sequence complementary SEQ ID NO:2 under conditions of high stringency, and confers resistance to cycloheximide at a concentration higher than 1 mg/ml in Kluyveromyces lactis, provided that said protein or fragment thereof confers resistance to cycloheximide at a concentration higher than or equal to 100 μg/ml when said sequence is introduced into a eukaryotic host cell under conditions allowing expression of said protein.
 3. The protein according to claim 1 obtained from Kluyveromyces lactis.
 4. A purified cycloheximide resistance protein comprising SEQ ID NO:
 1. 5. A purified protein which is specifically recognized by antibodies directed against a cycloheximide resistance protein, wherein said cycloheximide resistance protein comprises SEQ ID NO:1. 